Name: performing double fluorescence in situ hybridization to detect gene expression in mouse brain sections
Uploaded: 2025-04-28T12:01:16.000+00:00
Duration: 1 min 30 s
Description: Source: Jolly, S., et.al. Combining Double Fluorescence In Situ Hybridization with Immunolabelling for Detection of the Expression of Three Genes in Mouse ...

performing double fluorescence in situ hybridization to detect gene expression in mouse brain sections

Performing Double Fluorescence In Situ Hybridization to Detect Gene Expression in Mouse Brain Sections

Dilute the two probes in hybridization buffer, pre-warmed to 65 degrees Celsius, and mix well. Apply 300 microliters of hybridization mixture onto each slide, and cover with an oven baked coverslip. Subsequently, incubate the slides overnight at 65 degrees Celsius in a humidified chamber.The next day, transfer the slides into a Coplin jar containing pre-warmed wash buffer, and wash the slides for 30 minutes, twice at 65 degrees Celsius. After that, wash the slides for 10 minutes three times with MABT wash solution at room temperature.In this step, use a hydrophobic pen to draw circles around the tissue sections. Then, incubate the slides for one hour at room temperature with ISH blocking buffer in a humidified chamber. Next, incubate the slides overnight at 4 degrees Celsius with a horseradish peroxidase-conjugated anti-FITC antibody.Then, place the slides into a Coplin jar containing PBST. Wash them in PBST three times for 10 minutes each time, and replace with fresh PBST each time. Afterward, add fluorescent tyramide to the slides, and leave them for 10 minutes at room temperature. Place the slides into a Coplin jar, and wash in PBST for 10 minutes three times.Subsequently, incubate the slides with ISH blocking buffer for one hour at room temperature. Then, incubate the slides overnight at 4 degrees Celsius with an alkaline phosphatase conjugated anti-DIG antibody. After that, wash them with MABT three times for 10 minutes each time. Next, wash the slides twice with 0.1 molar Tris-HCL at pH 8.2 for five minutes at room temperature.Filter the fast red solution, and incubate the slides at 37 degrees Celsius with fast red solution in a humidified chamber. As the time for optimal development varies, check the slides regularly with a fluorescent microscope to monitor the formation of precipitate. Then, wash them three times with PBST for 10 minutes each time.

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 Performing Double Fluorescence In Situ Hybridization to Detect Gene Expression in Mouse Brain Sections

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.&#160;&#160;1. Hybridization<ol><li>Prepare 65 &#176;C wash buffer: 150 mM NaCl, 15 mM Na3C3H5O(COO)3 (= 1x saline sodium citrate), 50% (v/v) formamide and 0.1% (v/v) Tween-20.</li><li>Prepare MABT buffer: 100 mM maleic acid, 150 mM NaCl, 0.1% (v/v) Tween-20, pH 7.5.</li><li>Dilute the two probes (DIG-labelled and FITC-labelled) 1/1,000 in hybridization buffer (DEPC-treated deionized water with 50% (v/v) deionized formamide, 200 mM NaCl, 5 mM EDTA, 10 mM Tris-HCl pH 7.5, 5 mM NaH2PO4, 5 mM Na2HPO4, 0.01 mg/ml yeast tRNA, 1&#215; Denhardt's solution, and 10% w/v dextran sulfate) pre-warmed to 65 &#176;C and mix well.</li><li>Apply around 300 &#181;l of hybridization mixture onto each slide, coverslip with oven-baked (200 &#176;C) coverslips and incubate O/N at 65 &#176;C in a humidified chamber.</li><li>Transfer the slides into a Coplin jar containing pre-warmed wash buffer. Wash the slides for 30 min twice at 65 &#176;C with wash buffer.</li><li>Wash the slides for 10 min three times with MABT at RT.&#160;</li></ol>2. Visualization of the FITC Probe<ol><li>Prepare ISH blocking buffer: MABT with 2% blocking reagent and 10% heat-inactivated sheep serum.</li><li>Optional: use a hydrophobic pen to draw circles around the tissue sections on the slide to reduce the volume of antibody solutions required.</li><li>Incubate the slides for 1 hr at RT with ISH blocking buffer in a humidified chamber.</li><li>Incubate the slides O/N at 4 &#176;C with a horseradish peroxidase (POD)- conjugated anti-FITC antibody diluted 1/500 (v/v) in ISH blocking buffer.</li><li>Place the slides into a Coplin jar containing PBS with 0.1% (v/v) Tween-20 (PBST). Wash 3 times for 10 min in PBST and replace with fresh PBST each time.</li><li>Immediately before use, prepare the fluorescent tyramide by diluting 100 times into the Amplification diluent. For this example, use FITC-tyramide.</li><li>Add this to the slides and leave for 10 min at RT.</li><li>Place the slides into a Coplin jar and wash 3 times in PBST for 10 min.</li></ol>3. Visualization of the DIG Probe<ol><li>Prepare 0.1 M Tris- HCl pH 8.2.</li><li>Incubate the slides with ISH blocking buffer for 1 hr at RT.</li><li>Incubate the slides O/N at 4 &#176;C with an alkaline phosphatase (AP) -conjugated anti-DIG antibody diluted 1/1,500 (v/v) in ISH blocking buffer.</li><li>Wash with MABT for 10 min three times.</li><li>Wash twice with 0.1 M Tris-HCl pH 8.2 for 5 min at RT.</li><li>Immediately before use, prepare Fast Red solution by dissolving the tablets in 0.1 M Tris pH 8.2. Filter the solution through a 0.22 &#181;M filter.</li><li>Incubate the slides at 37 &#176;C with Fast Red solution in a humidified chamber. As the time for optimal development varies, check the slides regularly with a fluorescent microscope to monitor the formation of precipitate. For this example, stop the reaction after 2 - 3 hr.</li><li>Wash with PBST for 10 min three times.</li></ol>

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 performing double fluorescence in situ hybridization to detect gene expression in mouse brain sections

<a href='https://app-jove-com.remotexs.ntu.edu.sg/v/53976/combining-double-fluorescence-situ-hybridization-with-immunolabelling'>Source: Jolly, S., et.al. Combining Double Fluorescence In Situ Hybridization with Immunolabelling for Detection of the Expression of Three Genes in Mouse Brain Sections. J. Vis. Exp. (2016).</a>This video demonstrates the use of double fluorescence in situ hybridization to visualize the expression of two RNA targets in mouse brain sections. The protocol involves sequential detection of RNA using probes labeled with fluorescein isothiocyanate and digoxigenin, followed by enzymatic signal amplification to enhance sensitivity. The resulting fluorescence enables co-localization analysis of the target RNAs within the tissue.

Source: Jolly, S., et.al. Combining Double Fluorescence In Situ Hybridization with Immunolabelling for Detection of the Expression of Three Genes in Mouse ...

Take a chemically-fixed mouse brain section.Add a hybridization mixture containing a permeabilization agent and RNA probes labeled with FITC or DIG.Incubate to allow cell permeabilization and probe entry.The probes bind to complementary sequences on MBP mRNA, a reference marker ubiquitously expressed in oligodendrocytes, or ASPA mRNA, the target.Wash to remove unbound probes.Add a blocking buffer to prevent non-specific antibody binding.Introduce HRP-conjugated anti-FITC antibodies targeting the FITC-labeled probe.Wash, then add FITC-tyramide.HRP oxidizes FITC-tyramide into a highly reactive form that binds to nearby proteins, amplifying the fluorescence signal.Wash and reintroduce the blocking buffer.Add alkaline phosphatase-conjugated anti-DIG antibodies targeting the DIG-labeled probe.Wash and apply the Fast Red solution.Alkaline phosphatase dephosphorylates Fast Red, producing a fluorescent precipitate.Visualize under a fluorescence microscope.Co-localization of Mbp and ASPA signals indicates ASPA expression in oligodendrocytes.

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비디오: Performing Double Fluorescence In Situ Hybridization to Detect Gene Expression in Mouse Brain Sections - 실험

Quantitative Analysis of Alternative Pre-mRNA Splicing in Mouse Brain Sections Using RNA In Situ Hybridization Assay

Alternative splicing (AS) occurs in more than 90% of human genes. The expression pattern of an alternatively spliced exon is often regulated in a cell type-specific fashion. AS expression patterns are typically analyzed by RT-PCR and RNA-seq using RNA samples isolated from a population of cells. In situ examination of AS expression patterns for a particular biological structure can be carried out by RNA in situ hybridization (ISH) using exon-specific probes. However, this particular use of ISH has been limited because alternative exons are generally too short to design exon-specific probes. In this report, the use of BaseScope, a recently developed technology that employs short antisense oligonucleotides in RNA ISH, is described to analyze AS expression patterns in mouse brain sections. Exon 23a of neurofibromatosis type 1 (Nf1) is used as an example to illustrate that short exon-exon junction probes exhibit robust hybridization signals with high specificity in RNA ISH analysis on mouse brain sections. More importantly, signals detected with exon inclusion- and skipping-specific probes can be used to reliably calculate the percent spliced in values of Nf1 exon 23a expression in different anatomical areas of a mouse brain. The experimental protocol and calculation method for AS analysis are presented. The results indicate that BaseScope provides a powerful new tool to assess AS expression patterns in situ.

Quantitative Analysis of Alternative Pre-mRNA Splicing in Mouse Brain Sections Using RNA In Situ Hybridization Assay

An in situ hybridization (ISH) protocol that uses short antisense oligonucleotides to detect alternative pre-mRNA splicing patterns in mouse brain sections is described.

대체 사전 mRNA 접합 교 잡 시험 현장에서 RNA를 사용 하 여 마우스 뇌 섹션에서의 정량 분석

Alternative splicing (AS) occurs in more than 90% of human genes. The expression pattern of an alternatively spliced exon is often regulated in a cell ...

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JoVE Journal

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Localization of Odorant Receptor Genes in Locust Antennae by RNA In Situ Hybridization

Insects have evolved sophisticated olfactory reception systems to sense exogenous chemical signals. These chemical signals are transduced by Olfactory Receptor Neurons (ORNs) housed in hair-like structures, called chemosensilla, of the antennae. On the ORNs&#39; membranes, Odorant Receptors (ORs) are believed to be involved in odor coding. Thus, being able to identify genes localized to the ORNs is necessary to recognize OR genes, and provides a fundamental basis for further functional in situ studies. The RNA expression levels of specific ORs in insect antennae are very low, and preserving insect tissue for histology is challenging. Thus, it is difficult to localize an OR to a specific type of sensilla using RNA in situ hybridization. In this paper, a detailed and highly effective RNA in situ hybridization protocol particularly for lowly expressed OR genes of insects, is introduced. In addition, a specific OR gene was identified by conducting double-color fluorescent in situ hybridization experiments using a co-expressing receptor gene, Orco, as a marker.

Localization of Odorant Receptor Genes in Locust Antennae by RNA In Situ Hybridization

This paper describes a detailed and highly effective RNA in situ hybridization protocol particularly for low-level expressed Odorant Receptor (OR) genes, as well as other genes, in insect antennae using digoxigenin (DIG)-labeled or biotin-labeled probes.

RNA에 의한 Locust Antenna 내의 악취 수용체 유전자의 국산화<em&gt; 현장에서</em&gt; 하이브리드 화

Insects have evolved sophisticated olfactory reception systems to sense exogenous chemical signals. These chemical signals are transduced by Olfactory ...

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Visualization of SARS-CoV-2 using Immuno RNA-Fluorescence In Situ Hybridization

This manuscript provides a protocol for in situ hybridization chain reaction (HCR) coupled with immunofluorescence to visualize severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) RNA in cell line&#160;and three-dimensional (3D) cultures of human airway epithelium. The method allows highly specific and sensitive visualization of viral RNA by relying on HCR initiated by probe localization. Split-initiator probes help amplify the signal by fluorescently labeled amplifiers, resulting in negligible background fluorescence in confocal microscopy. Labeling amplifiers with different fluorescent dyes facilitates the simultaneous recognition of various targets. This, in turn, allows the mapping of the infection in tissues to better understand viral pathogenesis and replication at the single-cell level. Coupling this method with immunofluorescence may facilitate better understanding of host-virus interactions, including alternation of the host epigenome and immune response pathways. Owing to sensitive and specific HCR technology, this protocol can also be used as a diagnostic tool. It is also important to remember that the technique may be modified easily to enable detection of any RNA, including non-coding RNAs and RNA viruses that may emerge in the future.

Here, we describe a simple method that combines RNA fluorescence in situ&#160;hybridization (RNA-FISH) with immunofluorescence to visualize severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) RNA. This protocol may increase understanding of the molecular characteristics of SARS-CoV-2 RNA-host interactions at a single-cell level.

시투 혼성화에서 면역 RNA-형광을 이용한 SARS-CoV-2의 시각화

This manuscript provides a protocol for in situ hybridization chain reaction (HCR) coupled with immunofluorescence to visualize severe acute respiratory ...

Performing Double Fluorescence In Situ Hybridization to Detect Gene Expression in Mouse Brain Sections

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Performing Double Fluorescence In Situ Hybridization to Detect Gene Expression in Mouse Brain Sections